Metabolic fate of N,N-dimethyl-N′-(p-phenoxyphenyl)sulfamide in Rat, Dog, and Human

Metabolic Fate of N,N-Dimethyl-N'-(p -phenoxyphenyl)sulfamide in Rat, Dog, and Human F. F. S U N X and J. E. STAFFORD

Abstract The patterns of urinary excretion products of N,Ndimethyl-N'-(p-phenoxypheny1)sulfamide(I) in the rat, dog, and human have been examined. After oral administration, the drug was extensively metabolized in all species and the amount of intact drug excreted in the urine was negligible ( < l % ) . The metabolic pathways were via hydroxylation of the phenoxy ring, Ndemethylation, O-methylation, and conjugation. The following metabolites have been identified in free and/or conjugated form: N-methyl-N'-(p-phenoxypheny1)sulfamide (11). N,N-dimethylN'-p-(4-hydroxyphenoxy)phenylsulfamide (III), N,N-dimethylN'-p-(2-hydroxyphenoxy)phenylsulfamide (IV), N-methyl-N'-p(4-hydroxyphenoxy)phenylsulfamide (V), N-methyl-N'-p-(2-hydroxyphenoxy)phenylsulfamide (VI), N,N-dimethyl-N'-p-(4-hydroxy-3-methoxyphenoxy)phenylsulfamide (VII), and N-methylN'-p-(4-hydroxy-3-methoxyphenoxy)phenylsulfamide (VIII). The major differences in the patterns of urinary metabolites were: ( a ) the monomethyl (11) was the major metabolite in the dog and human but a minor one in the rat, ( b ) the para-hydroxylated compound (111) was the major metabolite in the rat, (c) hydroxylation of the phenoxy ring in the ortho-position (IV and VI) was observed in the rat and dog but not in the human, and ( d ) the methoxylated compound (VII) was found only in rat urine. K e y p h r a s e s N, N-Dimethyl-N'-(pphenoxypheny1)sulfamideurinary excretion after oral administration, metabolic pathways, rat, dog, man Urinary excretion-metabolites of N,N-dimethylN'-(p-phenoxyphenyl)sulfamide, oral administration, rat, dog, man Metabolism, N,N-dimethyl-N'-(p-phenoxypheny1)sulfamide-urinary products after oral administration, rat, dog, man

N,N-Dimethyl- N' -(p-phenoxypheny1)sulfamidel (I) reduces cholesterol levels significantly in both tyloxapol*-treated and cholesterol-cholic acid-fed rats (1). It has no significant effect on the cholesterol levels in normal rats and dogs. TLC analyses indicated that the drug was extensively metabolized. The results from studies designed to characterize the metabolism of I in the rat, dog, and human are reported here. EXPERIMENTAL Dosage an d Collection of Samples-Rat-Micronized I was suspended in 0.25% methylcellulose in sterile water3 with a glass Teflon homogenizer. The suspension was administered via oral intubation to six Sprague-Dawley rats (three males and three females) at a dose level of 100 mg/kg. A second group of six rats (three males and three females) that received the vehicle only served as the control. The rats were dosed daily for 21 days. Urine samples were collected daily, pooled, and kept frozen until analyzed. Dog-Four dogs, participating in chronic toxicity studies, had received daily oral doses of 100 mg/kg I for approximately 10 months. Urine samples were collected by catheterization a t 4-8 hr after administration of the drug. Urine samples were also obtained from untreated animals. Human-Four subjects each received a single 500-mg oral dose

of I in hard-filled capsules. Urine samples were collected from -12 to 0 and from 0 to 24 hr after drug administration. The postadministration urine for each subject was pooled. Urine collected prior to drug administration was used as the control. Extraction an d Purification-Aliquots of the urine samples (150-200 ml) were acidified to pH 3.5 with acetic acid and extracted six times with a n equal volume of chloroform. The chloroform layers were separated, pooled, and concentrated under reduced pressure. Residual chloroform in the extracted urine specimens was removed a t 45" under reduced pressure (1 hr). The p H of the urine was adjusted to 5.0 with 1 M sodium acetate buffer (pH 5.0), and 1/100 volume of a concentrated 8-glucuronidase aryl sulfatase solution4 was added; the mixture was then incubated a t 37" for 24 hr. The hydrolysis mixture was acidified to pH 3.5 and extracted three times with an equal volume of chloroform. The extracts were pooled and concentrated under reduced pressure. The control urine samples were processed in the same manner. The concentrated extracts were streaked a t the origin across three-fourths of the width of a 2-mm thick silica gel G-254 preparative TLC plates. The corresponding control urine extract was streaked on the remaining one-fourth of the width of the plate. The plate was developed in a solvent system of chloroform-methanol (95:5). To obtain good resolution, the plate was developed, dried, and redeveloped three to five times. After development was completed, the chromatogram was visualized with a 254-nm UV lamp. Zones that were present in the urine extracts from drug-treated subjects but not in the controls were scraped off the plate and eluted with chloroform-methanol (9:1). The purified extracts were evaporated to dryness. The residues were dissolved in a small amount of ethanol-free chloroform for introduction into the gas chromatograph6-mass spectrometer. Identification of Metabolites-Identification of the urinary metabolites of I was carried out by using mass spectrometry, IR spectroscopy, and, when possible, NMR spectroscopy. Mass spectrometric analysis was routinely carried out as follows: 5 pl of a sample and 2 p1 of bis(trimethylsily1)acetamide were injected simultaneously into the gas chromatograph-mass spectrometer. A 1.21-m (4-ft) column of 1%SE-30 (methylpolysiloxy gum) on Gas Chrom Q was maintained a t 210". The mass spectrometer was operated a t an ionization potential of 70 ev with an ion-source temperature of 290". On-column silylation was selected for simplicity and conservation of material. Unless the metabolite being studied was contaminated with large amounts of urinary impurities, the on-column silylation technique generally provided a completely silylated derivative of the compound. IR and NMR analyses were carried out without silylation. IR spectra were obtained with a ~pectrophotometer~ and micro KBr pellets containing 50-100 pg of the sample. Since the NMR analysiss required 3-5 mg of sample, it was done only when that amount of material was available. TLC Characterization of I Metabolites -Specific spray reagents were used to detect the phenolic and nonphenolic metabolites on the thin-layer chromatograms. Phenolic metabolites appeared immediately as a pink spot on the plate when sprayed with either of the following two reagents: ( a ) a freshly mixed 1:l solution of 0.5% (w/v) aqueous ferric chloride and 0.5% (w/v) methanolic dipyridyl, and ( b ) a freshly mixed 1 : l solution of 0.5%

5

V-25,030. Triton WR-1339. Upjohn Vehicle 122.

Sigma type H-2 8-glucuronidase No. G-0876. 143,000 units/ml Brinkmann.

LKB-9000. Perkin-Elmer model 421. 8Varian XL-100.

Vol. 63, No. 4, April 1974 / 539

183

TMS 0 I

100 @@J-

I'

0

75

364 M +

,C"3

II

s - N,

CH3

163

50

25

0

50

100

200

150

250

400

350

300

mle

Figure 1-Mass

spectrum of trimethylsilyl derivative of I .

benzidine in 0.17 M HC1 and 10% aqueous sodium nitrite. These sprays were also used to detect any drug-related compounds obscured by other UV-absorbing materials present in the chromatographed urine extracts.

tive of I. The fragmentation peaks a t 163 and 164 indicated that the aromatic system was not modified. The most prominent peak in the spectrum was a t m / e 198. Precise mass measurement gave the empirical formula of C ~ ~ H I ~ (calc. N O 198.09189, found 198.09142). These results suggested that a methyl from one tri-

RESULTS AND DISCUSSION Isolation and characterization studies of the urinary excretion products of I indicated extensive metabolism (Scheme I) of the drug in animals and humans. The metabolites were present in the urine mainly as glucuronide and/or sulfate conjugates. A summary of all detectable drug-related compounds found in the urine of I-treated rats, dogs, and humans is presented in Table I. A metabolic map, based on this information, is presented in Scheme I. Combined GLC-mass spectrometry were used extensively to determine the structure of the metabolites. The mass spectrum of the trimethylsilyl derivative of I is presented in Fig. 1. The drug shows a strong molecular ion peak a t m / e 364. Cleavage between the aniline and sulfamoyl group (M-108) gave another peak at 256. In the metabolism studies, the mass of these two fragments provided important information of N-demethylation pathways. The free phenoxyaniline ions appeared a t m / e 183 and 184. Further fragmentation of the phenoxyaniline part of the molecule gave mass peaks a t 163 and 164, which served as indicators of any metabolic modifications in the aromatic system. Negligible amounts of unchanged drug were found in the urine specimens from animals and humans. In the rat and dog, the presence of trace amounts of the unchanged drug could be demonstrated only by GLC-mass spectrometric analysis. The relative amounts of each metabolite excreted were estimated from the size of the peaks on the gas chromatogram (Fig. 2). Evidence for the identification of the major metabolites is summarized below. The common mass peaks appearing in the mass spectra of I-related compounds are presented in Table 11. N-Methyl-N'-@-phenoxypheny1)sulfamide (11)-This compound is the N-demethylation product of I found in the urine of the dog and human in unconjugated form. It was also found in the urine of the rat but only in trace amounts. The mass spectrum of the N,N'-bis(trimethylsily1) derivative of I1 is shown in Fig. 3. The molecular ion was a t m / e 422. Loss of the sulfamoyl group (M - 166) showed the material to be the desmethyl deriva-

Table I S u m m a r y of All Drug-Related Compounds F o u n d in the Urine of Rat, Dog, and Human

Com pound

I 11 111 IV

v

VI VII VIII

Co n -

Free j u g a t e d +

++

+

+-

-

-

++ ++ ++

8

7

6

W

$5 0

a

v)

W

Lz

4

3

2

Urine in which Compound Was Found

F o r m of Exc r e t io n ~

~

Rat

Dog

Human

Trace Trace

Trace

Trace

++ ++ ++

+++ ++

++++

(11) R t = 1.6 MIN

9

1

:t 1

2

3

4

5

6

7

8

RETENTION TIME, rnin

Figure 2-Gas-liquid chromatogram of p-glucuronidase aryl sulfatase hydrolyzed (37' for 24 hr) human urine extrmt. Vol. 63, No. 4, April 1974 J 541

100

75 50

1

198 (M-224)

I 100

50

150

200

250

300

350

400

450

m/e

Figure 3-Mass

100 7 75

spectrum of bis (trimethylsilyl) derivative of

II. TMS

I

TMSO

G O a k -!-N,

-

1

TMS 0

loo

-kN:CH3

-I OTMS

163

methylsilyl group migrated to the phenoxyaniline system upon electron impact. This unique property was shared by all desmethyl I-related compounds (Metabolites V, VI, and VIII). Both IR and UV spectra of I1 were identical to unchanged I. The chromatographic and spectroscopic characteristics of 11, synthesized independently, were identical with the isolated material. The hypolipidemic activity of I1 was equivalent to the parent, I. N , N-Dimethyl-” - p - (4-hydroxyphenoxy)phenylsulfamide (111)-This metabolite was found both free and conjugated in the urine of all three species. The mass spectrum of the bis(trimethylsily1) derivative (Fig. 4) showed a molecular ion at m / e 452. Loss of 108 indicated that the sulfamoyl group was intact. The presence of the 163 and 164 pair indicated that the hydroxyl substitution did not affect the cleavage between the phenoxy oxygen and the aniline ring. Loss of the trimethylsilyl group from the aniline nitrogen and the loss of trimethylsilanol from the phenoxy ring gave strong mass peaks at m / e 271 and 181. UV spectra of 111 were obtained in 95% ethanol and also with the addition of base (0.1 N KOH). In the absence of base, the spectrum showed a strong band a t 238 nm and a weak band at 282 nm, which was similar to the parent compound (238, 270, and 278 nm). In the presence of 0.1 N KOH, the strong band was shifted to 252 nm and the weak band was shifted to 299 nm. The intensity of both bands was increased. The behavior was consistent with a monohydric phenol (4). The IR spectrum showed

542/Journal of Pharmaceutical Sciences

CH3

271

50 -

75

,CH3

6

CH3

344 (M-108)

bands at 1295 and 1270 cm-1 which were phenol C-0 vibrations. The features of the aromatic system and the sulfamoyl group of the parent compound were preserved. The assignment of the hydroxyl group to the para-position of the phenoxy ring was confirmed by NMR. The spectrum showed two sets of AA’BB’ multiplets, which indicated that all aromatic substitutions were para. On the thin-layer plate, Ill gave a strong positive response when sprayed with bipyridyl-ferric chloride reagent or benzidine reagent, which indicated the presence of the phenolic functional group. Compound 111, synthesized independently, had identical chromatographic and spectroscopic characteristics to the isolated material. The hypolipidemic activity of I11 was also equivalent to the parent, I. N , N - Dimethyl-” - p - (2-hydroxyphenoxy)phenylsulfamide (1V)-This compound was found by its distinct chromatographic behavior both by TLC and GLC. Compound IV migrated more rapidly on silica gel G-254 than did 111 and had a n R, value very close to 11. Compounds I1 and IV were distinguished from each other by spraying the plate with bipyridyl-ferric chloride reagent; IV appeared as a pink spot, whereas I1 remained colorless. Upon GLC, the trimethylsilyl derivative of IV (retention time 1.8 min) emerged much faster than the corresponding derivative of I11 (retention time 4.4 min). The mass spectrum (Fig. 5) of the bis(trimethylsilyl) derivative of IV showed the molecular ion a t m / e 452, identical with its 4-isomer. The fragmentation pattern of IV

TMS 0 100

CHJO

15 50 25

0

h 50

100

200

150

250

300

350

400

450

500

m/e

Figure 6- M a s s spectrum of bis (trimethylsilyl) derivative of V I I . was similar to 111 except for the lack of the 163 and 164 pair, which indicated that a metabolic modification had occurred in the proximity of the oxygen between the two phenyl rings. The NMR spectrum of IV could not be factored with certainty because the eight aromatic hydrogens form two highly coupled sets that were overlapping. One set of the multiplet was identified as an AA'BB' pattern, indicating that one phenyl ring had symmetrical para-para substitution. Thus, the possibility of hydroxylation on the aniline ring was ruled out. Hydroxylation in the metaposition relative t o the phenoxy oxygen was unlikely because of the unfavorable inductive effect. Therefore, the hydroxyl group in IV was assigned to the ortho-position. The IR spectra of 111 and IV were similar. Compound IV was found in both free and conjugated forms in the urine of the rat and dog only. It was not found in human urine during the 24 hr after drug administration. N-Methyl-N'-p-(4-hydroxyphenoxy)phenylsulfamide (V)The N-desmethyl-4-hydroxy metabolite, both free and conjugated, was found in the urine of all three species. The mass spectrum of the trimethylsilyl derivative showed that the molecular ion was a t m / e 510. Fragments a t m / e 344 ( M - 166) and 286 (M - 244) were characteristic of N-demethylated I. The presence of the 163 and 164 pair suggested that the hydroxyl substitution was not ortho to the phenoxy oxygen. Loss of trimethylsilanol was indicative of the relation of V with 111. The presence of a phenolic hydroxyl group in V was established by its UV spectra, reactivity with bipyridyl-ferric chloride reagent, and NMR spectrum. The UV spectrum taken in a neutral ethanol solution resembled that of the parent drug (238 and 282 nm). When the spectrum was redetermined a t alkaline pH, a

Table 11-Common

bathochromic shift of both bands to 252 and 298 nm, respectively, was observed, as was found for 111, which suggested the presence of a monohydric phenol. NMR spectra showed two sets of AA'BB' multiplets, suggesting that all aromatic substitutions were para. The IR spectrum was also consistent with the structure assignment. N-Methyl-N'-p-(2-hydroxyphenoxy)phenylsulfamide (V1)The metabolite was found in conjugated form in rat urine only. It was not isolated and its presence was established by GLC-mass spectrometric analysis of the partially purified extract containing 111 and VII. The mass spectrum of the trimethylsilyl derivative was identical to that of V except for the lack of the 163 and 164 pair. This suggested that VI was the 2-isomer of V (the N-demethylated analog of IV). On TLC, VI had a higher R, than V and reacted with bipyridyl-ferric chloride reagent to give a pink-colored spot. N,N -D i m e t hy I -N'-p-(4-hydroxy-3-methoxyphenoxy )phenylsulfamide (VI1)-Compound VII was a minor metabolite found only as a conjugate in rat urine. It had the same R, value as 111 on TLC but was separated from I11 by repeated TLC. The mass spectrum (Fig. 6) of the trimethylsilyl derivative showed a molecular ion a t m / e 482. Loss of 108 mass units indicated that the dimethyl sulfamoyl group was intact. Loss of the trimethylsilyl group from the aniline nitrogen (M - 72) followed by the loss of trimethylsilanol gave two prominent ions at 301 and 211. Presence of the 163 and 164 pair indicated that substitutions on the aromatic system were not in the close proximity .of the diphenyl ether oxygen. Loss of 30 (CH20) and 31 (CHBO)from all major peaks indicated the presence of a phenyl methyl ether linkage (5). Since the amount of this compound in the urine was very

Mass P e a k s Appearing in Mass S p e c t r a of I-Related C o m p o u n d s

mle

Structure

Appears in all spectra Appears in all spectra of phenolic compounds Appears in all spectra except IV a n d VI A p p e a r s in all phenolics A p p e a r s i n all phenolics Appears i n all phenolics Appears in I and I1 Appears i n I and I1 Appears i n all phenolics Appears i n I1 Appears in all N-desmethyl hydroxylated metabolites Appears in V I I I Appears in all s p e c t r a A p p e a r s in all metabolites w i t h methoxyl g r o u p Appears in all compounds w i t h sulfamide i n t a c t

73 75 163

90 180 271 256 185 344 198 286 316

M - 15 M - 30 or M -31 M - 108

LOSSof SOzN(CH3)z

M - 166 M - 224

Comments

Appears in all desmethyl metabolites

LOSSof SOzN

CH3

'

di(CH3), f r o m nitrogen

and trimethylsilyl

Appears in all desmethyl metabolites

Vol. 63, No. 4, April I974 I 5 4 3

small, it could not be isolated for further spectral analysis. Therefore, the positions of hydroxy and methoxy substitution on the aromatic system were assigned, based on the following information: (a) the presence of the 163 and 164 pair in the mass spectrum precluded the possibility of any substitution located ortho to the diphenyl ether oxygen; ( b ) the product of enzymatic hydroxylation of para-substituted monohydric phenols is catechol, which undergoes 0-methylation yielding para-substituted orthomethoxy phenol (6); and (c) catechol 0-methyltransferase does not 0-methylate resorcinol derivatives (7). N-Methyl-N’-p-(4-hydroxy-3-methoxyphenoxy)phenylsulfamide (VII1)-Compound VIII is the N-demethylation product of VII. It was found in the urine of all three species in conjugated form. The amount was very small but was separated from the crude urine extract by repeated TLC. The mass spectrum of VIII of the trimethylsilyl derivative showed that the molecular ion was at m/e 540. Loss of the N-trimethylsilyl-N-methylsulfamoyl group ( M - 166) and the appearance of the 4-hydroxy-3-methoxy-N-methylphenoxyaniline ion a t 316 ( M - 224) indicated a monomethyl sulfamide analog. Loss of 30 or 31 mass units suggested it was a methoxy phenol. Presence of the 163 and 164 pair indicated that the hydroxyl and methoxy substitutions were not ortho to the phenoxy oxygen. The NMR spectrum of VIII was difficult to interpret because of the overlapping of aromatic protons. However, a set of AA’BB’ multiplets indicated one phenyl ring had para-para symmetric disubstitution. This ruled out the possibility that the aniline ring was modified. Based on the same argument as for VII, VIII was assigned the structure of the N-demethyl-4-hydroxy-3-methoxy analog of the parent drug. In conclusion, the results of these experiments indicated that the metabolic fate of the parent drug was different in these three species. Rats can only demethylate the drug a t reduced efficiency, as shown by the presence of only trace amounts of I1 (the N -

demethylated product) and the presence of VII in rat urine. The lack of IV and VI (ortho-hydroxylated metabolites) in human urine may indicate that humans can only hydroxylate I in the paraposition. However, since the human subjects in this study were only administered a single dose of the drug while the animals were administered multiple doses, this apparent species variation may be caused by enzyme induction in animals. REFERENCES

(1) W.A. Phillips, P. E. Schurr, and N. A. Nelson, Fed. Proc., 29,385(1970). (2) G . M. Barton, J.Chromatogr., 20,189(1965). (3)J. Sherma and L. V. S. Hood, ibid., 17,307(1965). (4) A . I. Scott, “Interpretation of the Ultraviolet Spectra of Natural Products,” Macmillan, New York, N.Y., 1965,p. 95. (5) C. S. Barnes and J. L. Occolowitz, Aust. J. Chem., 16, 219(1965). (6) J. Daly, J. K . Inscoe, and J. Axelrod, J. Med. Pharm. Chem., 8.153(1965). (7) M. S. Masri, D. J. Robbins, 0. H. Emerson, and F. Deeds, Nature, 202,878( 1964). ACKNOWLEDGMENTS AND ADDRESSES Received February 26, 1973, from the Research Laboratories, The Upjohn Company, Kalamazoo, MI49001 Accepted for publication November 13,1973. The authors thank Dr. M. F. Grostic, Dr. G . Slomp, and Dr. W. C. Krueger and their assistants for spectral analyses and valuable discussions. They also thank Dr. T. Sawa for the supply of urine specimens from drug-treated dogs and Dr. D. Lednicer for supplying authentic I1 and 111. To whom inquiries should be directed.

Microbiological Synthesis of L-Dopa JOHN ROSAZZA*”, PAUL FOSSS, MICHAEL LEMBERGERS, and CHARLES J. SIHS

Abstract The ability of microorganisms to convert N-carbobenzoxyl-L-tyrosine, N-tert-butyloxycarbonyl-L-tyrosine,and N-formyl-L-tyrosine into their respective N-substituted L-dopa derivatives was studied. These tyrosine derivatives were examined because of the ease with which the blocking groups may be removed. L-Tyrosine derivatives were incubated with Aspergillus ochraceous or Gliocladium deliquescens, and the resulting L-dopa products were isolated and characterized. L-Dopa was metabolized by G. deliquescens to 3,4-dihydroxyphenylaceticacid and 3,4-dihydroxyphenethyl alcohol. L-Ascorbic acid and hydrocinnamic acid increased yields of L-dopa when added to fermenta-

Keyphrases L-Dopa-microbiological synthesis, L-tyrosine derivatives incubated with Aspergillus ochraceous and Cliocladium deliquescens, isolation and identification of L-dopa products Aspergillus ochraceow-used for microbiological synthesis of L-dopa products from L-tyrosine derivatives 0 Gliocladium deliquescensused for microbiological synthesis of L-dopa products from L-tyrosine derivatives Microbiology-synthesis of L-dopa from L-tyrosine by microorganisms Levodopa-microbiological synthesis of L-dopa from L-tyrosine derivatives

Three different types of enzymes are known to catalyze the formation of L-dopa from L-tyrosine: 1. Tyrosine hydroxylase is a n enzyme associated with the biosynthesis of norepinephrine. It catalyzes the tetrahydropteridine-dependenthydroxylation of L-tyrosine to L-dopa (1). 2. Tyrosinase catalyzes the oxidation of tyrosine to melanin. I t is generally accepted th at the reaction proceeds through t he formation of L-dopa an d hallo-

chrome, with the eventual formation of the polymeric pigment, melanin (2). 3 . P-Tyrosinase from Escherichia intermedia catalyzes the synthesis of L-dopa from L-tyrosine and pyrocatechol uia P-replacement ( 3 ) . In view of the therapeutic importance of L-dopa (levodopa) in the treatment of Parkinsonism, the authors wish to record in detail the examination of reactions using microbial systems for the conversion

544 1Journal of Pharmaceutical Sciences

tion media.